Antibodies to polypeptides encoded by aspartoacylase polynucleotides

ABSTRACT

Canavan disease, an autosomal recessive leukodystrophy, is caused by deficiency of aspartoacylase and accumulation of N-acetylaspartic acid in brain. Human aspartoacylase (ASP) cDNA spanning 1,435 bp has been cloned and expressed in  E. coli . A base change, a854&gt;c, has been found in 85% of the 34 Canavan alleles tested so far, which results in a missense glu285&gt;ala mutation that is predicted to be part of the catalytic domain of aspartoacylase. The invention therefore provides nucleic acid sequences, genes, polypeptides, antibodies, vectors containing the gene, host cells transformed with vectors containing the gene, animal models for the disease, methods for expressing the polypeptide, genetic screening methods and kits, diagnostic methods and kits, methods of treating Canavan disease and methods of genetic therapy for the disease.

This application is a continuation of U.S. application Ser. No. 09/965,807, filed Oct. 1, 2001, now U.S. Pat. No. 7,217,547 which is a continuation of U.S. application Ser. No. 08/128,020 filed Sep. 29, 1993, now abandoned both of which are incorporated by reference herein.

BACKGROUND OF THE INVENTION

Canavan disease (CD), or spongy degeneration of brain, is an autosomal recessive leukodystrophy associated with mental retardation, megalencephaly, hypotonia and death, usually in the first decade of life. Brain histology in CD is characterized by spongy degeneration of white matter with astrocytic swelling and elongated mitochondria¹⁻⁵. Canavan disease is more prevalent in Jewish people of Ashkenazi origin³⁻⁵. Matalon et al. (1988) described aspartoacylase deficiency as the basic biochemical defect in CD⁶. Since the initial report, 145 patients have been diagnosed with CD a single center, suggesting that CD is more prevalent than previously thought¹⁰⁻¹². Aspartoacylase deficiency in CD has also been reported by other investigators^(13,14).

The deficiency of aspartoacylase in CD leads to excessive excretion of NAA in urine and its accumulation in brain^(6,9-11). Aspartoacylase in brain has been localized to white matter associated with myelin tracks¹⁶. How aspartoacylase and the hydrolysis of NAA are involved in keeping white matter intact is not clear. It is also not understood how the deficiency of aspartoacylase leads to the pathogenesis seen in CD.

Aspartoacylase has been purified and characterized from bovine brain and from other bovine and human sources¹⁶. Biochemical and immunochemical studies suggest that aspartoacylase has been conserved during evolution. Aspartoacylase activity has been found in a variety of mammalian tissues, including kidney, brain white matter, adrenal glands, lung, liver and cultured skin fibroblasts. Brain grey matter and blood constituents do not have any detectable aspartoacylase activity (Kaul et al., unpublished studies).

Aspartoacylase specifically hydrolyses N-acetyl-L-aspartic acid (NAA) to aspartate and acetate^(7,8). Stereospecificity of aspartoacylase towards L-analog of NAA has been well documented. The D-analog of NAA acts as a weak inhibitor of NAA hydrolysis by aspartoacylase. Studies have suggested that the carbon backbone of NAA is involved in interaction with the substrate binding site of aspartoacylase; and that the substitutions at α and β carboxyl groups of aspartate moiety do not have any effect on hydrolysis of NAA by aspartoacylase¹⁶.

The diagnosis of CD is now routinely made by quantitation of NAA in urine and estimation of aspartoacylase activity in cultured skin fibroblast¹². The level of aspartoacylase activity found in direct chorionic villi cells or in cultured chorionic villi cells and amniocytes is about 2 orders of magnitude lower than that found in normal cultured skin fibroblasts. Due to the low aspartoacylase activity in chorionic villi cells and amniocytes, the prenatal diagnosis of CD using aspartoacylase assay is not satisfactory¹⁵.

Due to the devastating nature of this genetic disease, there is an urgent need for better diagnostic methods for early detection of the disease, both pre- and postnatally, and screening methods to detect genetic carriers of the disease to allow informed genetic counseling for prospective parents. Additionally, there is a critical need for an effective treatment, and even more preferably, a cure for the underlying biochemical defect.

SUMMARY OF THE INVENTION

The present invention discloses the isolation and expression of human ASP cDNA, and thus provides the gene and protein encoded by the gene. In particular, the invention provides an isolated nucleic acid molecule comprising:

-   -   (a) a nucleic acid sequence encoding a human aspartoacylase         polypeptide;     -   (b) a nucleic acid sequence complementary to nucleic acid         sequence (a); or     -   (c) a nucleic acid sequence at least 16 nucleotides in length         capable of hybridizing, under stringent hybridization         conditions, with one of said nucleic acid molecules (a) or (b).

More particularly, the invention provides a nucleic acid molecule described in (a), above, comprising:

-   -   (i) a DNA molecule having the DNA sequence of FIG. 1 (SEQ ID         NO: 1) from DNA position +1 to +891;     -   (ii) a DNA molecule encoding a normal human aspartoacylase         polypeptide having the amino acid sequence of FIG. 1 (SEQ ID         NO: 1) from amino acid position +1 to +313;     -   (iii) a DNA molecule having a sequence of a fragment of the DNA         sequence of FIG. 1 (SEQ ID NO: 1), or a sequence complementary         thereto, and including at least 16 sequential nucleotides;     -   (iv) a DNA molecule having a sequence of a fragment of the DNA         sequence of FIG. 1 (SEQ ID NO: 1) and including at least 16         sequential nucleotides, and which encodes a fragment of the         amino acid sequence of FIG. 1 (SEQ ID NO: 1); or     -   (v) a DNA molecule encoding an epitope of the amino acid         sequence of FIG. 1 (SEQ ID NO: 1) between positions +1 to +313,         and encoded by at least 18 sequential nucleotides.

In addition, the invention provides allelic or mutant versions of the above DNA molecules (i)-(v) wherein they are modified in at least one nucleotide position as compared with the sequence of FIG. 1 (SEQ ID NO: 1), corresponding to the sequence of a naturally-occurring allele of human aspartoacylase having an altered biological activity.

In another aspect, the invention provides an isolated normal aspartoacylase polypeptide capable of hydrolyzing N-acetyl-aspartic acid to aspartate and acetate. In particular, the invention provides a normal aspartoacylase polypeptide having the amino acid sequence of FIG. 1 (SEQ ID NO: 1) from amino acid position +1 to +313 as well as a mutant aspartoacylase polypeptide having either an altered ability of hydrolyze N-acetyl-aspartic acid to aspartate and acetate or incapable of hydrolyzing N-acetyl-aspartic acid to aspartate and acetate.

In another aspect of the invention, in view of the identification of a base change in the human ASP encoded aspartoacylase, which base change is present in 85% of Canavan alleles, the invention provides a means of identifying DNA sequences containing the mutation. Therefore, the invention additionally provides a means of diagnosing the disease in patients, and identifying carriers of the genetic defect. This aspect of the invention includes methods for screening a potential Canavan disease carrier or patient for the presence of an identified mutation and/or a different mutation in an aspartoacylase gene; for example:

hybridization assays, comprising

(a) isolating genomic DNA from said potential Canavan disease carrier or patient,

(b) hybridizing a DNA probe onto said isolated genomic DNA, said DNA probe spanning said mutation in said aspartoacylase gene, wherein said DNA probe is capable of detecting said mutation,

(c) treating said genomic DNA to determine the presence or absence of said DNA probe and thereby indicating the presence or absence of said aspartoacylase mutation;

restriction fragment length polymorphism assays, comprising

(a) isolating genomic DNA from said potential Canavan disease carrier or patient,

(b) determining the presence or absence of a restriction endonuclease site in the gene, the presence or absence of which thereby indicates the presence or absence of said aspartoacylase mutation;

PCR assays, comprising

(a) isolating genomic DNA from said potential Canavan disease carrier or patient,

(b) determining the mobility of heteroduplex PCR products in polyacrylamide gels, the mobility of which thereby indicates the presence or absence of said aspartoacylase mutation; and

immunoassays, comprising

(a) providing a biological sample of the subject to be screened; and

(b) submitting the sample to an assay for detecting in the biological sample the presence of a normal aspartoacylase gene, a mutant aspartoacylase gene, normal aspartoacylase polypeptide, mutant aspartoacylase polypeptide, or mixtures thereof.

In the above methods of screening (assays), either the presence of the normal or mutant aspartoacylase polypeptide or nucleic acid coding for said polypeptide can be detected. For each of the assays, kits are provided for carrying out the methods of the invention. These kits include nucleic acids, polypeptides and antibodies of the present invention, including fragments such as nucleic acid probes, oligopeptide epitopes and antibody fragments such as F(ab′)₂ fragments.

In related aspects of the invention, genetic constructs and methods for making the nucleic acids, polypeptides and antibodies of the invention are provided, including cloning vectors, host cells transformed with cloning vectors and hybridomas; pharmaceutical preparations containing normal polypeptides for administering to patients to provide therapy to replace the mutant polypeptide; nucleic acid constructs suitable for administering to patients to provide a (preferably permanent) genetic therapy; methods for making the nucleic acids, polypeptides and antibodies of the present invention, including fragments such as nucleic acid probes, oligopeptide epitopes and antibody fragments such as F(ab′)₂ fragments; and animals transformed with normal and mutant aspartoacylase genes to provide animal models for study of CD and related genetic diseases.

It will be appreciated by a skilled worker in the art that the identification of the genetic defect in a genetic disease, coupled with the provision of the DNA sequences of both normal and disease-causing alleles, provides the full scope of diagnostic and therapeutic aspects of such an invention as can be envisaged using current technology.

BRIEF DESCRIPTION OF THE DRAWINGS

Various other objects, features and attendant advantages of the present invention will be more fully appreciated as the same becomes better understood when considered in conjunction with the accompanying drawings, wherein:

FIG. 1 (SEQ ID NO: 1) depicts the nucleotide and predicted amino acid sequence of human ASP encoded transcript and protein. The cDNA is 1,435 bp and the initiator “atg” marks base 1 of coding sequence. The polyadenylation signal sequences are shaded. Also shown are the 18 base poly(A) tail. Amino acid sequence predicted from the human ASP cDNA is depicted as single letter code and initiator amino acid residue M is residue 1. There are several in frame termination codons present in human ASP cDNA upstream of the initiator atg codon. The potential N-glycosylation site is shown in bold type and marked by an asterisk (*). The numbers on left show amino acid residues while those on right are nucleotide base position.

SEQ ID NO: 1       TTGTAACAGA AAATTAAAAT ATACTCCACT CAAGGGAATT CTG TACTTTG CCCTTTTGGT    −99       AAAGTCTCAT TTACATTTCT AAACCTTTCT TAAGAAAATC GAATTTCCTT TGATCTCTCT    −39   1                                          −1   M   T   S   C   H   I        TCTGAATTGC AGAAATCAGA TAAAAACTAC TTGGTGAA ATG ACT TCT TGT CAC ATT    18   7       A   E   E   H   I   Q   K   V   A   I   F   G   G   T   H   G         GCT GAA GAA CAT ATA CAA AAG GTT GCT ATC TTT GGA GGA ACC CAT GGG     66  23       N   E   L   T   G   V   F   L   V   K   H   W   L   E   N   G         AAT GAG CTA ACC GGA GTA TTT CTG GTT AAG CAT TGG CTA GAG AAT GGC    114  39       A   E   I   Q   R   T   G   L   E   V   K   P   F   I   T   N         GCT GAG ATT CAG AGA ACA GGG CTG GAG GTA AAA CCA TTT ATT ACT AAC    162  55       P   R   A   V   K   K   C   T   R   Y   I   D   C   D   L   N         CCC AGA GCA GTG AAG AAG TGT ACC AGA TAT ATT GAC TGT GAC CTG AAT    210  71       R   I   F   D   L   E   N   L   G   K   K   M   S   E   D   L         CGC ATT TTT GAC CTT GAA AAT CTT GGC AAA AAA ATG TCA GAA GAT TTG    258  87       P   Y   E   V   R   R   A   Q   E   I   N   H   L   F   G   P         CCA TAT GAA GTG AGA AGG GCT CAA GAA ATA AAT CAT TTA TTT GGT CCA    306 103       K   D   S   E   D   S   Y   D   I   I   F   D   L   H   N*  T         AAA GAC AGT GAA GAT TCC TAT GAC ATT ATT TTT GAC CTT CAC AAC ACC    354 119       T   S   N   M   G   C   T   L   I   L   E   D   S   R   N   N         ACC TCT AAC ATG GGG TGC ACT CTT ATT CTT GAG GAT TCC AGG AAT AAC    402 135       F   L   I   Q   M   F   H   Y   I   K   T   S   L   A   P   L         TTT TTA ATT CAG ATG TTT CAT TAC ATT AAG ACT TCT CTG GCT CCA CTA    450 151       P   C   Y   V   Y   L   I   E   H   P   S   L   K   Y   A   T         CCC TGC TAC GTT TAT CTG ATT GAG CAT CCT TCC CTC AAA TAT GCG ACC    498 167       T   R   S   I   A   K   Y   P   V   G   I   E   V   G   P   Q         ACT CGT TCC ATA GCC AAG TAT CCT GTG GGT ATA GAA GTT GGT CCT CAG    546 183       P   Q   G   V   L   R   A   D   I   L   D   Q   M   R   K   M         CCT CAA GGG GTT CTG AGA GCT GAT ATC TTG GAT CAA ATG AGA AAA ATG    594 199       I   K   H   A   L   D   F   I   H   H   F   N   E   G   K   E         ATT AAA CAT GCT CTT GAT TTT ATA CAT CAT TTC AAT GAA GGA AAA GAA    642 215       F   P   P   C   A   I   E   V   Y   K   I   I   E   K   V   D         TTT CCT CCC TGC GCC ATT GAG GTC TAT AAA ATT ATA GAG AAA GTT GAT    690 231       Y   P   R   D   E   N   G   E   I   A   A   I   I   H   P   N         TAC CCC CGG GAT GAA AAT GGA GAA ATT GCT GCT ATC ATC CAT CCT AAT    738 247       L   Q   D   Q   D   W   K   P   L   H   P   G   D   P   M   F         CTG CAG GAT CAA GAC TGG AAA CCA CTG CAT CCT GGG GAT CCC ATG TTT    786 263       L   T   L   D   G   K   T   I   P   L   G   G   D   C   T   V         TTA ACT CTT GAT GGG AAG ACG ATC CCA CTG GGC GGA GAC TGT ACC GTG    834 279       Y   P   V   F   V   N   E   A   A   Y   Y   E   K   K   E   A         TAC CCC GTG TTT GTG AAT GAG GCC GCA TAT TAC GAA AAG AAA GAA GCT    882 295       F   A   K   T   T   K   L   T   L   N   A   K   S   I   R   C         TTT GCA AAG ACA ACT AAA CTA ACG CTC AAT GCA AAA AGT ATT CGC TGC    930 311       C   L   H   .         TGT TTA CAT TAG AA ATCACTTCCA GCTTACATCT TACACGGTGT CTTACAAATT     984      CTGCTAGTCT GTAAGCTCCT TAAGAGTAGG GTTGTGCCTT ATTCAACTGC ATACATAGCT    1044      CCTAGCACAG TGCCTTATTC GGTAGGCATC TAAGCAAATT TCTTAAATTA ATTAATATAT    1104      CTTTAAAGAT ATCATATTTT ATGTATGTAG CTTATTCAAA GAAGTGTTTC CTATTTCTAT    1164      ATAGTTTATT ATACATGATA CTTGGGTAGC TCAACATTCT T

CAG CCTTTGTATT    1224      CAGAA

ATTGAAATA GATATATATA AAGTTAAAAA AAAAAAAAAA AAA           1277

FIG. 2 depicts the alignment of human (HLASP) and bovine (BASPCON) ASP encoded protein sequence using the AALIGN program (Gap penalty 4, Deletion penalty 12, PAMfile STANDARD.PAM) in Lasergene software package from DNAstar (Madison, Wis.). The human and bovine aspartoacylase amino acid sequences share 92.3% identity in 313 aa overlap. Consensus amino acid sequence motifs predicted to be involved in catalytic center of aspartoacylase are shown as shaded areas. The potential N-glycosylation site is marked by an asterisk (*), and phosphorylation sites are highlighted as shadows.

FIG. 3 depicts an autoradiogram of Northern blot analysis of poly(A)⁺ RNA isolated from various human tissues. Two μg of poly(A)⁺ RNA from each tissue were fractionated on agarose gel and blotted on nylon membrane and blots were hybridized to human cDNA under stringent conditions. The human poly(A)⁺ RNAs are from; 1: heart, 2: brain, 3: placenta 4: lung, 5: liver, 6: skeletal muscle and 7: kidney.

FIG. 4 depicts a schematic representation of pHLASP cloned in pBluescript SK⁻. The human ASP cDNA was cloned between Eco RI and Xho I sites in 5′→3′ direction and the transcription was driven by LACZ promoter. The initiator “atg” and terminator “tag” codons are shown. Other vector regions are not represented in the schematics. The figure is not drawn to scale.

FIG. 5 depicts the nucleotide sequence of 312 bp cDNA fragment in the region of a854>c mutation from normal controls (WT, Panel A) and a patient with CD (MUT, Panel B). Reverse transcription of cytoplasmic RNA with HKRT1 (AACCCTACTCTTAAGGAC; SEQ ID NO: 5) primer was followed by amplification with HASP14F (F→CCGGGATGAAAATGGAGAA; SEQ ID NO: 6) and HASPC7R (R→ACCGTGTAAGATGTAAGC; SEQ ID NO: 7) primers. The prefix F and R in these oligos stand for M13 universal and reverse primer tags. Fluorescent di-deoxy sequencing of both strands were carried out with M13 universal and reverse primers. The patient with CD (MUT) was homozygous for a854>c point mutation and the base involved is shown by a down arrow (.dwnarw.). The mutation would result in E285>A missense mutation at the amino acid level.

FIG. 6 depicts the single strand conformation polymorphism (Panel A) and Eag I restriction endonuclease digestion (Panel B) of 237 bp cDNA fragment amplified by RT-PCR of cytoplasmic RNA from normal controls, and Canavan probands and their family members. After initial reverse transcription of cytoplasmic RNA with HKRT1 (AACCCTACTCTTAAGGAC; SEQ ID NO: 5) primer the 237 bp cDNA fragment was amplified using HASPG5 (AGGATCAAGACTGGAAACC; SEQ ID NO: 8) and HASPC7 (GTAAGACACCGTGTAAGA TG; SEQ ID NO: 9) primers. Representative SSCP and restriction digestion analysis of a854>c point-mutation in 3 families is shown and the pedigrees are drawn at the top. One of the normal controls (Lane 4) and the non-carrier sibling of a patient with CD (Lane 1) are also shown.

FIG. 7 is a restriction map of the structural gene sequences of ASP.

GENERAL DISCUSSION

The discovery of aspartoacylase deficiency and N-acetylaspartic aciduria has for the first time offered a definite diagnosis for CD without the need for brain biopsy (for review, see Matalon et al., 1993)¹². The spongy degeneration of white matter in CD strongly suggests that hydrolysis of NAA by aspartoacylase plays a significant role in the maintenance of intact white matter.

Canavan disease is the only known genetic disorder which is caused by a defect in the metabolism of a small metabolite, NAA, synthesized exclusively in the brain^(22,23) in a cell specific manner²⁴⁻²⁶. Since the initial discovery of NAA in brain²⁷, its biological role has remained unknown²⁸⁻³². The stable level of NAA in brain has made it a useful marker in ¹H NMR spectroscopy of brain (for review, see Birken and Oldendorf, 1989)³³. Significantly reduced levels of NAA have been reported in non-CD focal or generalized demyelinating disorders³⁴, Huntington disease³⁵, HIV-seropositive individuals³⁶, acute stroke³⁷, myodystrophic mice³⁸ and mouse model of scrapie³⁹. While such decrease in NAA level has been proposed as a measure of neuronal loss, it is not specific for any particular pathology. The accumulation of NAA, and dystrophy of white matter, in brain of patients with CD is highly specific and the elevated NAA level has been demonstrated both by biochemical and as well as ¹H NMR spectroscopy of brain^(9,10,16,34).

Aspartoacylase is present in a variety of tissues, and in most of the tissues tested, (Kaul et al., unpublished studies). Northern blot analysis has confirmed the expression of human ASP in the tissues tested so far. However, the enzyme seems to have a unique role in maintaining a homeostatic balance of NAA level, particularly in the white matter of brain. The disturbance of this equilibrium, as seen in CD, somehow leads to spongy degeneration of the white matter. The pathology seen in CD is apparently co-localized to the regions of brain that express aspartoacylase activity¹⁶. The grey matter, despite several fold increased levels of NAA¹⁶, is spared of any significant pathological changes in CD. Without wishing to be bound by theory, it is believe that the critical role of NAA in brain function and biology is manifested through the action of aspartoacylase.

Since the pathology in CD is observed only in brain, it is suggested that aspartoacylase in tissues other than brain acts as scavenger of NAA from body fluids. The relative abundance of two human ASP transcripts is apparently regulated in a tissue dependent manner. The choice of polyadenylation site, and/or alternative splicing of pre-mRNA, as reason for the two transcripts is plausible. The polyadenylation signal or/and alternative splicing may provide an additional mode of regulating gene expression²⁰.

Hydrolysis of NAA by aspartoacylase is highly specific. N-Acetyl derivatives of amino acids other than aspartic acid are not hydrolyzed by aspartoacylase. In contrast, NAA is not hydrolyzed by aminoacylase I, an enzyme that hydrolyzes N-acetyl derivatives of all other amino acid, including N-acetyl-L-glutamic acid^(7,8).

Human ASP encoded transcript and protein apparently do not share any homology with the human aminoacylase I cDNA.sup.21. Human and bovine aspartoacylase have sequences that have homology to the catalytic domain sequence motifs reported in esterases and other related hydrolytic enzymes.sup.19. The invariable amino acid residues histidine (H) and glutamic acid (E) involved in catalysis by esterases are present in the consensus sequence motifs GGTHGNE (SEQ ID NO: 10) and VNEAAYY (SEQ ID NO: 11) in aspartoacylase. The inhibition of aspartoacylase activity by diisopropyl fluorophosphate, (Kaul, unpublished data), further suggests that a serine (S) amino acid residue is involved at the active site. It is therefore proposed that aspartoacylase has an esterase-like activity and that its catalytic domain involves a triad of S, H and E amino acid residues. The E285 amino acid residue in wild type aspartoacylase is indeed part of the VXEXXXY (SEQ ID NO: 12) sequence motif involved in catalysis by esterases, and is conserved in bovine aspartoacylase. The substitution of the amino acid residue E with A residue should lead to the inactivation of aspartoacylase, as is observed in CD in patients with E285>A mutation.

The mutation data is based on a sample of 17 unrelated pedigrees of Ashkenazi Jewish descent. Since a854>c base change in ASP has not been observed in any of the 168 normal chromosomes analyzed, it supports the conclusion that this base change is indeed a mutation causing CD. The apparently predominant nature of a854>c point mutation, detected in 85% of the Canavan alleles, further suggests a founder effect of this mutation in the Jewish population. Such a predominant mutation can facilitate the study of epidemiology of CD in the population at risk. Mutation analysis can also be used for reliable screening for carriers of the genetic defect, as well as prenatal diagnosis.

In addition, two other mutations in the ASP gene have been identified which are also associated with Canavan disease:

One is a c693>a mutation, which results in the codon change TAC>TAA, which results in a translation error of Y231>X; thus, this mutation causes premature termination of the polypeptide chain at the location where a tyrosine residue is supposed to be. This is a “nonsense” mutation.

Another allele which has been identified is a c914>a change, which results in the codon change GCA>GAA, which in turn results in the missense mutation A305>E, substituting a glutamic acid for an alanine residue.

Thus, several mutations have been identified which are involved in Canavan disease, including a missense mutation which has been localized in the predicted catalytic domain of aspartoacylase, indicating the underlying genetic defect in the disease in the majority of patients. Therefore, the present invention also provides methods of treating and curing Canavan disease, comprising administering therapeutically effective amounts of a biologically active protein or a biologically active fragment thereof, or drugs which overcome the biological deficit caused by the genetic defect (the pharmacological approach), or administering therapeutically effective amounts of a nucleotide sequence coding for a biologically active protein or a biologically active fragment thereof, which nucleic acid allows the production of a biologically effective aspartoacylase protein in the affected cells (the genetic therapy approach).

In the disclosure which follows, it will be appreciated by the skilled worker that implementing the various utilities disclosed herein, as well as others, which can be derived from the provision of the DNA sequence for aspartoacylase of present invention, e.g., screening of carriers, diagnosis of disease and therapeutic applications, including polypeptide and gene therapies, are routinely achievable in view of the guidance of this disclosure, as well in view of conventional knowledge. Thus, the numerous routine protocols for conducting these various applications are also well known. Thus, for example, various other genes which are implicated in genetic defects are disclosed in the prior art, as are examples of various utilities for these other genes, and the genes, polypeptides, antibodies, etc., of the present invention, can be prepared analogously; similarly, the methods of the present invention can be conducted analogously.

DEFINITIONS

As used herein, “aspartoacylase” means the polypeptide coded for by the ASP gene, e.g., in humans. This definition thus includes the protein as isolated from human or animal sources, as produced by recombinant organisms and as chemically or enzymatically synthesized according to techniques routine in the art. This definition is understood to include the various polymorphic forms of the polypeptide wherein amino acid substitutions in the non-critical or variable regions of the sequence do not affect the essential functioning of the polypeptide or its secondary or tertiary structure. This definition includes the polypeptide which, in its normal condition, is present in non-Canavan disease patients or carriers and wherein it performs its normal functions.

As used herein, “mutant aspartoacylase” or “allelic variant of aspartoacylase” or “Canavan aspartoacylase” means the polypeptide coded for by an ASP gene which is highly analogous to aspartoacylase in terms of primary, secondary and tertiary structure, but wherein one or more amino acid substitutions, and/or deletions and/or insertions result in impairment of its essential function, so that organisms whose brain white matter cells express mutant aspartoacylase rather than normal aspartoacylase demonstrate one or more symptoms of Canavan disease.

As used herein, “Canavan disease” or “CD” refers to the genetic disease autosomal recessive leukodystrophy, defined above.

As used herein, “CD carrier” means a person in apparent health whose chromosomes contain a mutant ASP gene that may be transmitted to that person's offspring.

As used herein, “CD patient” means a person who carries a mutant ASP gene on both chromosomes on which the gene is carried, such that they exhibit the clinical symptoms of Canavan disease.

As used herein, “ASP gene” refers to the gene whose mutant forms are associated with Canavan disease. This definition is understood to include the various sequence polymorphisms that exist, wherein nucleotide substitutions in the gene sequence do not affect the essential function of the gene product. This term primarily relates to an isolated coding sequence, but can also include some or all of the flanking regulatory elements and/or any introns.

As used herein, “stringent hybridization conditions” are defined in accordance with what a skilled worker would understand such conditions to mean, depending on the nucleic acids being hybridized. Thus, stringent hybridization conditions for DNA-DNA hybrids are different from those for DNA-RNA heteroduplexes, and conditions for short (e.g., less than 200 and especially under 100 nucleotides in length) oligonucleotides are generally different than those for long sequences (≧200 nucleotides). Suitable conditions meeting the requirement of stringency are described in Reference 45. For example, for short oligonucleotide sequences, stringent conditions generally include hybridization at temperatures 5-10° C. below the T_(m) for the specific sequence.

As used herein, “an aspartoacylase having altered biological activity” means an aspartoacylase polypeptide having a biological activity which, when expressed in vivo, results in phenotypic effects or symptoms of Canavan disease.

As used herein, “complementary” means a nucleic acid molecule has a sequence which complements a reference template sequence, whereby the two sequences can specifically hybridize. Preferably, the term refers to exact complementarity, e.g., as is found between the two strands of a nucleotide sequence in a naturally-occurring gene.

It will be understood by those of skill in the art that allelic or other sequence variations in the DNA and amino acid sequences of the ASP gene and its product aspartoacylase are included in the present invention. For example, allelic variants which result in aspartoacylase polypeptides having the identical amino acid sequence to the normal or most prevalent variant due to degeneracy of the genetic code are included. Further, allelic variants which result in aspartoacylase having essentially insignificant changes in the non-critical or variable regions of the polypeptide, e.g., not in regions of the polypeptide involved in the biological activity of the polypeptide such as is seen in Canavan disease, are also considered to be equivalents included in the scope of this invention. Such variants include those resulting in amino acid substitutions, e.g., as shown in Table 1, which provide a polypeptide having essentially the same function as the normal polypeptide. In each individual case, the equivalency can be determined by measuring the biological activity of the polypeptide in comparison with the normal polypeptide, e.g., according to the assay described in Reference 16. In contrast, it is more likely that sequence variations which occur inside the consensus sequences described below for esterase catalytic sites, which variations result in amino acid sequences not fitting the consensus sequence, will in turn result in a polypeptide with altered biological activity.

TABLE 1 Generally Equivalent Substitution of Amino Acids in a Polypeptide Original Amino Acid Equivalent Amino Acid Ala Gly, Ser Arg Lys Asn Gln, His Asp Glu Cys Ser Gln Asn Glu Asp Gly Ala, Pro His Asn, Gln Ile Leu, Val Leu Ile, Val Lys Arg, Gln, Glu Met Leu, Tyr, Ile Phe Met, Leu, Tyr Ser Thr Thr Ser Trp Tyr Tyr Trp, Phe Val Ile, Leu

In general, the functions or the immunological identity may be significantly changed if substituents are selected which are less conservative than the amino acids shown in Table 1. Such significant changes can be achieved by substitutions with amino acids which differ more in their structure and in the functional groups. Significant changes are those having an effect on the three-dimensional structure, e.g., wherein the pleated sheet structure or the helical structure is affected. Also, interactions of the charged and the hydrophobic chains can be affected.

Mutations are defined by the homology of two polypeptides which are compared. The term “homology” comprises similar amino acids (for example, Table 1) and gaps in the sequences of the amino acids (homology=similarity). The polypeptides according to the invention have an amino acid sequence which has a homology of at least 80%, preferably 90%, more preferably 95% and most preferably 98% of the amino acid sequence of FIG. 1 (SEQ ID NO: 1).

As previously mentioned, the invention also comprises modifications of the DNA or cDNA. These modified sequences hybridize under stringent conditions with the DNA, which codes the protein according to the invention. The cDNA or DNA has a nucleotide sequence, which has a homology of at least 70%, preferably 80%, more preferably 90% and most preferably 95% with the cDNA or DNA sequence according to the FIG. 1 (SEQ ID NO: 1). The homology can be measured by hybridization, as it is described in R. Knippers, Molekulare Genetik (Molecular Genetics), 1982, Third Edition, Georg Thieme Verlag Stuttgart, New York.

The invention also includes polypeptides having posttranslational modifications, which are to be understood to mean changes which occur during or after translation. These include glycosylation, formation of disulfide bridges, and chemical modifications of the amino acids, for example, sulfation.

Glycosylation is a basic function of the endoplasmic reticulum and/or the Golgi apparatus. The sequence and the branching of the oligosaccharides are formed in the endoplasmic reticulum and changed in the Golgi apparatus. The oligosaccharides can be N-linked oligosaccharides (asparagine-linked) or O-linked oligosaccharides (serine-, threonine- or hydroxylysine-linked). The form of glycosylation is dependent on the host cell type and on the type from which the corresponding cell type is derived. The extent and the type of glycosylation can be affected by substances, for example as described in European publication EP 0 222 313. The variation of glycosylation can change the function of the protein.

Proteins often form covalent bonds within the chains. These disulfide bridges are produced between two cysteines, whereby the protein is specifically pleated. Disulfide bridges stabilize the three-dimensional structure of the proteins.

Methods for Isolating, Cloning and Expressing the ASP Gene

The methods used to isolate, clone and express the ASP gene disclosed in FIG. 1 (SEQ ID NO: 1) are outlined in Examples 1-6, below. However, it is evident to a skilled worker that, given the DNA sequence provided herein, many other means of isolating this gene and other related sequences, e.g., from other humans, including those having allelic variations of the sequence of FIG. 1 (SEQ ID NO: 1), e.g., from other libraries, including cDNA libraries from other human tissues as well as genomic libraries, from other species, including those from existing cDNA and genomic libraries as well as those which are commercially available or can be routinely constructed, e.g., according to methods well known in the art, e.g., according to the methods outlined in Sambrook et al.⁴⁵, are additionally made available. For example, probes synthesized in accordance with the DNA sequence in FIG. 1 (SEQ ID NO: 1) can be used to screen libraries constructed from the DNA isolated from other individuals or other species to find corresponding genes. In particular, given the conserved nature of the gene determined by sequence comparison with the bovine ASP gene, the almost ubiquitous presence of aspartoacylase in many tissue types tested thus far and the ubiquitous presence of NAA in other mammals, it is likely that many other animals contain an equivalent gene.

In general terms, the production of a recombinant form of aspartoacylase can be effected by a wide variety of procedures well known to those of ordinary skill in the art. In particular, the recombinant polypeptide can be produced following the procedures outlined in U.S. Pat. No. 5,227,292 for the neurofibromatosis type 1 gene and protein, especially from column 6, line 12 to column 8, line 2 and references cited therein (the disclosures of which are incorporated by reference herein), except that the procedures are conducted starting with a DNA encoding and aspartoacylase gene instead of an NF1 gene. Suitable promoters, control sequences, vectors, host cells, etc. are routinely determinable, e.g., as disclosed in WO 91/02796, directed to analogous methods for isolation, cloning and expressing the gene for cystic fibrosis, in particular, e.g., from page 95, line 28 to page 100, line 29 and the references cited therein. In particular it is noted that both normal and mutant polypeptides can be produced.

Thus, in view of the disclosure herein of the sequence for the aspartoacylase gene and suitable probes for the gene, aspartoacylase genes can be isolated from any suitable source and routinely be cloned into a suitable cloning vector, and ultimately into an expression vector, i.e., a replicable vector suitable for transforming a host cell and containing the aspartoacylase DNA sequence in operable linkage with suitable control sequences whereby the DNA sequence can be expressed. (Definitions of the terms used in this section, e.g., “operable linkage”, “control sequences”, etc., have their usual meanings, e.g., as described in U.S. Pat. No. 5,227,292, as well as in WO 93/06244.) The vector is then used to transform a suitable host cell and the host cell is cultured under suitable conditions to effect expression of the DNA sequence into the corresponding polypeptide. The expressed polypeptide is then isolated according to standard techniques well known in the art.

Methods for Isolating the Aspartoacylase Polypeptide

A method for isolating aspartoacylase from bovine brain is outlined in Reference 16, which isolation procedure is fully applicable to other aspartoacylase polypeptides from other tissues in which it is expressed. However, it is evident to a skilled worker, given the ability to produce the cloned aspartoacylase polypeptides in recombinant expression systems of the present invention, that purification from such expression systems can be performed analogously to other purifications from such sources, given the physicochemical properties of the polypeptide, e.g., properties which are revealed by its sequence as disclosed by the present invention, and the teaching of, e.g., Reference 16, as well as utilizing routine experimentation for optimization of results, e.g., yields and activity, from a particular source. For example, WO 91/02796 discloses methods for selecting purification techniques based upon the properties of the polypeptide. Other such techniques are well known in the art. For final purification of the polypeptide, many standard techniques can be utilized, e.g., ion exchange chromatography, gel permeation chromatography, adsorption chromatography or isoelectric focusing, immuno-affinity chromatography (see the discussion regarding preparation of antibodies to aspartoacylase), preparative polyacrylamide gel electrophoresis, and high performance liquid chromatography (HPLC).

The homogeneity of the thus-produced aspartoacylase can be determined using standard protein analytical techniques. See, e.g., Sambrook et al.⁴⁵

Preparation of Antibodies to Aspartoacylase

The present invention also provides antibodies which selectively bind to epitopes of aspartoacylase. These antibodies can be produced according to well known techniques in the art, including immunization of suitable antibody-producing animals with whole aspartoacylase polypeptides (including the mutant forms of aspartoacylase) or immunologically-effective fragments thereof, e.g., epitopes, to provide polyclonal antibodies to the polypeptide. Preferably, the antibodies are high affinity antibodies, e.g., having affinities, i.e., dissociation constants, of 10⁻⁶, more preferably 10⁻⁷, 10⁻⁸, 10⁻⁹ or higher. In addition, according to well known techniques such as, e.g., Kohler and Milstein⁴⁹, monoclonal antibodies to epitopes of aspartoacylase can also be produced. Still further, antibody fragments, such as F(ab′)₂ fragments, can be produced and used according to well known methods.

These antibodies or antibody fragments can be used for a variety of purposes. For example, they can be used to purify aspartoacylase from solutions, e.g., fractionated cell supernatants or media containing secreted aspartoacylase from host cells containing the clones gene in an expressible, secreted form. Additionally, the antibodies, or fragments thereof, can be used in a wide variety of immunological assays for the detection of aspartoacylase and its mutants. Thus, these antibodies can be used in the immunoassay-based screening and diagnostic methods of the present invention.

Treatment by Administration of Functional ASP Protein or Fragments Thereof

In a pharmacological approach, treatment of Canavan disease can be performed by replacing the defective aspartoacylase polypeptide with normal polypeptide, by modulating the function of the defective polypeptide or by modifying another step in the pathway in which aspartoacylase participates in order to correct the physiological abnormality.

To be able to replace the defective polypeptide, reasonably large amounts of pure aspartoacylase must be available. Pure aspartoacylase can be obtained as described above from cultured cell systems, e.g., containing cloned and expressed ASP gene. Delivery of the polypeptide to the affected white matter requires its packaging and administration by means which allows the intact polypeptide to cross the blood-brain barrier, e.g., by disrupting the barrier, thereby allowing the polypeptide to pass through it, e.g., according to the methods outlined in U.S. Pat. No. 4,866,042 and references cited therein, or by encapsulating the polypeptide in, e.g., liposomes, whereby the barrier can be crossed without disruption, e.g., according to the methods outlined in WO 91/04014 and references cited therein. Other techniques known in the art for delivery to the affected situs can also be used.

Suitable amounts of polypeptide and regimens of administration, including routes and frequency of administration, for treatment of Canavan disease can be routinely determined by the skilled practitioner. For example, an effective dosage for treatment of a patient who has been diagnosed with Canavan disease will be 0.1 to 100 U/kg, more preferably 0.5 to 60 U/kg, still more preferably 1 to 20 U/kg, most preferably 2 to 10 U/kg of body weight/day, or twice weekly, and which will be optimized for the individual patient, e.g., in analogy with administration of glucocerebrosidase for treatment of Gaucher disease. Optimization of dosage can be determined by monitoring clinical symptoms, as well as measuring the levels of NAA in various body tissues. For example, NMR spectroscopy of the brain can be used to monitor NAA levels in vivo. Effective dosages are those which substantially alleviate the clinical manifestations of Canavan disease.

The aspartoacylase polypeptide can be formulated in conventional ways standard in the art for administration of protein substances. Administration by injection with a pharmaceutically acceptable carrier or excipient, either alone or in combination with another agent, is preferred. Suitable formulations include solutions or suspensions emulsions or solid compositions for reconstitution into injectables. Acceptable pharmaceutical carriers are those which dissolve the aspartoacylase polypeptide or hold it in suspension and which are not toxic to the extent of permanently harming the patient. Those skilled in the art will know, or be able to ascertain with no more than routine experimentation, particular suitable pharmaceutical carriers for this composition. See, for example, the protocols disclosed in U.S. Pat. No. 5,227,292 (see, e.g., column 12, line 1-68).

Treatment by Genetic Therapy

In a preferred therapeutic aspect of the present invention, patients suffering from Canavan disease are provided with a permanent source of normal aspartoacylase polypeptide, i.e., by way of provision of a normal ASP gene, at the appropriate site(s) in the body to partially, substantially or totally relieve the deleterious effects of the genetic defect in the mutant ASP gene. Such somatic gene therapy has been shown to be effective for a number of genes involved in genetic defects. For example, adenosine deaminase deficiency disease has been cured by administration of a normal gene for the defective enzyme. Similarly, the gene coding for aspartoacylase is provided to patients in need of such treatment, i.e., patients suffering from Canavan disease, whereby the deleterious effects of the defective mutant gene are relieved.

Various options are available for effecting genetic therapy, including but not limited to somatic gene therapy at the affected site, e.g., administering a therapeutically effective dosage of the gene to tissues and/or cells in which the gene is needed to prevent disease; whole body somatic therapy, whereby most if not all tissues and/or cells in the body receive a therapeutically effective dosage of the gene, whether or not the disease is manifested in that tissue or cell; and germ line gene therapy, wherein the genetic defect is cured in the reproductive cells of the carrier or patient, whereby that person will only transmit normal and not defective alleles to his or her children.

The preferred gene therapy method for Canavan disease will vary with the patient or carrier to be treated, and can be determined using no more than routine experimentation by the skilled practitioner. In particular, guidance a gene therapy techniques and considerations are disclosed in the series Human Gene Therapy⁵⁰. Introduction of the DNA coding for the normal aspartoacylase into cells in need of this treatment can be through the use of retroviral vectors, non-retroviral vectors such as adenoviral vectors, vaccinia virus herpesvirus, or animal virus vectors such as Moloney murine leukemia virus and SV40 virus. Protocols for such gene therapy are disclosed in WO 91/02796 (page 106, line 15-page 108, line 9), as well as those disclosed in WO 92/10564 and WO 90/11092. Particular protocols can be optimized as needed.

The methods of delivery of the genetic therapeutic material to a particular location, e.g. the white matter of the brain, are also disclosed in the various references cited herein, and in particular in U.S. Pat. No. 4,866,042 and references cited therein, and in WO 91/04014 and references cited therein.

Other Treatments

Other treatment regimes can also be facilitated by the present invention. For example, drug therapy providing modulation of the defective aspartoacylase can be developed by using screening methods made possible by the present invention. Cultured cell systems expressing the defective aspartoacylase polypeptide can be used to screen drugs for their effectiveness in vitro for improving the performance of the defective polypeptide. Alternatively, drugs can be designed based upon the disclosed structure of the polypeptide to compensate for the defective structure of the mutant polypeptide. Still further, drugs could be developed which modulate the stability or production of the defective polypeptide in order to compensate for the decreased activity of the mutant polypeptide. These alternatives are discussed in detail in WO 91/02796 with respect to the cystic fibrosis polypeptide, which discussion is fully applicable herein to the aspartoacylase polypeptide.

In addition, the present invention facilitates the development of therapies based on modulation of the amounts of substrate and/or end products of the reaction catalyzed by aspartoacylase. For example, acetate and/or aspartic acid and/or their further metabolites may be administered to compensate for the lack of production of these products, including their further metabolic products, e.g., analogously to the administration of L-DOPA to compensate for the deficiency of tyrosine hydroxylase in Parkinsonism. Alternatively, if the clinical symptoms are caused by excessive buildup of NAA, compounds can be administered to bind, e.g, chelate, NAA, or to competitively inhibit its binding at sites where such binding is causing the clinical symptoms, e.g., analogously to administration of dopamine antagonists in the treatment of amphetamine and drug abuse.

Production of Probes and Primers

Various aspects of the present invention require the use of nucleotide probes and primers which hybridize with nucleic acid sequences of the aspartoacylase gene. Given the sequence of that gene provided herein, it is routine for such molecules to be prepared. See, e.g., the manufacturer's instructions which accompany various commercial PCR amplification equipment and kits (e.g., those of Perkin Elmer Cetus), or nucleic acid synthesizers (e.g., those of Applied Biosystems, Inc., Foster City, Calif.).

Design and selection of suitable probes and primers is routine for the skilled worker. For example, suitable probes for detecting a given mutation include the nucleotide sequence at the mutation site and encompass a sufficient number of nucleotides to provide a means of differentiating a normal from a mutant allele. Suitable probes include those complementary to either the coding or noncoding strand of the DNA. Similarly, suitable PCR primers are complementary to sequences flanking the mutation site. Production of these primers and probes can be carried out in accordance with any one of the many routine methods, e.g., as disclosed in Sambrook et al.⁴⁵, and those disclosed in WO 93/06244 for assays for Goucher disease.

In general, suitable probes and primers will comprise, at a minimum, an oligomer at least 16 nucleotides in length, since, as disclosed in Reference 45 (page 11.7), calculations for mammalian genomes indicate that for an oligonucleotide 16 nucleotides in length, there is only one chance in ten that a typical cDNA library (complexity≈10⁷ nucleotides) will fortuitously contain a sequence that exactly matches the sequence of the nucleotide. Therefore, suitable probes and primers corresponding to epitopes are generally 18 nucleotides long, which is the next larger oligonucleotide fully encoding an amino acid sequence (i.e., 6 amino acids in length).

Methods of Pre- and Postnatal Diagnosis and Carrier Screening

By use of nucleotide and polypeptide sequences provided by the present invention, safe, effective and accurate testing procedures are also made available to identify carriers of mutant alleles of aspartoacylase, as well as pre- and postnatal diagnosis of fetuses and live born patients carrying either one or two mutant alleles. This affords potential parents the opportunity to make reproductive decisions prior to pregnancy, as well as afterwards, e.g., if chorionic villi sampling or amniocentesis is performed early in pregnancy. Thus, prospective parents who know that they are both carriers may wish to determine if their fetus will have the disease, and may wish to terminate such a pregnancy, or to provide the physician with the opportunity to begin treatment as soon as possible, including prenatally. In the case where such screening has not been performed, and therefore the carrier status of the patient is not known, and where Canavan disease is part of the differential diagnosis, the present invention also provides a method for making the diagnosis genetically, without resort to brain biopsy.

Many versions of conventional genetic screening tests are known in the art. Several are disclosed in detail in WO 91/02796 for cystic fibrosis, in U.S. Pat. No. 5,217,865 for Tay-Sachs disease, in U.S. Pat. No. 5,227,292 for neurofibromatosis and in WO 93/06244 for Goucher disease. Thus, in accordance with the state of the art regarding assays for such genetic disorders, several types of assays are conventionally prepared using the nucleotides, polypeptides and antibodies of the present invention. For example:

Genetic screening: Biological samples containing nucleic acids can be evaluated using a variety of nucleic acid-specific techniques:

1. Direct sequencing: The DNA from an individual can be cloned, whereby both alleles are cloned. They can then be evaluated for differences in their nucleic acid sequence from normal alleles by direct sequencing of the individual's aspartoacylase gene.

2. Heteroduplex analysis: RNA transcripts can be made from a standard cloned gene, either the normal or mutant gene, and then hybridized with DNA from the individual and the resulting heteroduplex treated with RNase A and run on a denaturing gel to detect the location of any mismatches.

3. Restriction Fragment Length Polymorphism (RFLP): Restriction enzymes can be used which provide a characteristic pattern of restriction fragments, wherein a restriction site is either missing or an additional restriction site is introduced in the mutant allele. Thus, DNA from an individual and from control DNA sequences are isolated and subjected to cleavage by restriction enzymes which are known to provide restriction fragments which differentiate between normal and mutant alleles, and the restriction patterns are identified. While this assay is very simple, it is limited by the requirement that the mutation being tested for is known in advance.

4. Single Strand Conformation Polymorphism (SSCP): This is a rapid and sensitive assay for nucleotide alterations, including point mutations. See Reference 42. DNA segments 100-400 bp in length are amplified by PCR, heat denatured and electorphoresed on high resolution, non-denaturing acrylamide gels. Under these conditions, each single-stranded DNA fragment assumes a secondary structure determined in part by its nucleotide sequence. Even single base changes can significantly affect the electrophoretic mobility of the PCR product.

5. Polymerase Chain Reaction (PCR): This powerful technique can be used to test very small amounts of DNA from an individual, by amplifying DNA sequences in the region flanking the portion of the aspartoacylase gene known to be involved in a given mutation. Sequencing or other analysis of the amplified sequences is thereby simplified.

Polypeptide Screening:

1. Enzymatic activity: Biological samples from the individual to be tested e.g., taken from tissues in which detectable levels of aspartoacylase are normally produced, are assayed for the presence of aspartoacylase. It is noted that brain samples are not required, even though the effects of the mutant gene are most profound in white matter. The presence or absence of an enzymatically effective aspartoacylase can then be detected according to the assay outlined in Reference 16.

2. Immunoassay: Antibodies can be produced which are specific for either or both normal or mutant aspartoacylase, according to methods outlined above. Biological samples from the individual to be tested are then assayed, e.g., taken from tissues in which detectable levels of aspartoacylase are normally produced. It is noted that brain samples are not required, even though the effects of the mutant gene are most profound in white matter. A variety of immunoassays can then be performed on the samples, using a variety of detection methods, to detect the presence or absence of the mutant gene product.

Details of protocols for performing these screening techniques are well known in the art, and are exemplified in WO 91/02796 and references cited therein, as well as U.S. Pat. No. 5,217,865, which details analogous techniques for screening for Tay-Sachs disease, which, coincidentally, is a genetic disease also present in the Ashkenazi Jewish population. Therefore, assay methods and kits are also provided which can be used to simultaneously screen for these two, as well as other, genetic diseases.

Animal Models for Canavan Disease

The creation of a mouse or other animal model for Canavan disease is crucial to a full understanding of the disease and to test possible therapies (for a review of creating animal models, see Erickson⁵¹). Currently, no animal model of Canavan disease exists. The evolutionary conservation of the aspartoacylase gene as demonstrated by the sequence homology with the bovine gene indicates that an orthologous gene is likely to exist in the mouse, which can be identified using human or bovine aspartoacylase sequences as probes. Thereby, generation of a specific mutation analogous to the Canavan allele can be effected to reproduce the disease phenotype, as well as other mutations, including complete inactivation of the mouse gene, in order to study the biochemistry, molecular biology and physiology of the polypeptide.

For making such animal models, the various methods disclosed in WO 91/02796 can be adapted for the aspartoacylase gene with only routine experimentation.

Thus, in addition to providing materials for screening, treatments and diagnoses, the present invention provides materials which are useful as research tools, e.g., in order to further investigate basic questions regarding the role of aspartoacylase in Canavan disease, as well as other genetic disease caused by, e.g., mutations in enzymes, in particular esterases, as well as the role of NAA hydrolysis by aspartoacylase in the disease and lead to better management of patients with CD.

Without further elaboration, it is believed that one skilled in the art can, using the preceding description, utilize the present invention to its fullest extent. The following preferred specific embodiments are, therefore, to be construed as merely illustrative and not limitative of the remainder of the disclosure in any way whatsoever.

In the foregoing and in the following examples, all temperatures are set forth uncorrected in degrees Celsius; and, unless otherwise indicated, all parts and percentages are by weight.

The entire disclosures of all applications, patents and publications, cited above and below, if any, are hereby incorporated by reference; the attached appendices are a part of this specification, and references cited therein are also hereby incorporated by reference.

EXAMPLES Part I: Materials and Methods Example 1 Materials, Reagents and Bacterial Strains

The materials and reagents used in the study were: Immobilon PVDF transfer membrane (Millipore, Bedford, Mass.); restriction enzymes (IBI, New Haven, Conn.; New England Biolabs, Beverly, Mass., Promega, Madison, Wis. and Boehringer Mannheim, Indianapolis, Ind.); Gene Amp RNA PCR kit and AmpliTaq PCR kit for amplification of DNA (Perkin-Elmer Cetus, Norwalk, Conn.); Random primed DNA labeling kit (Boehringer Mannheim, Indianapolis, Ind.); α-[³²P]-dNTP's, 3000 Ci/mMole (NEN/Dupont, Wilmington, Del.); RNAzolB kit for preparation of cytoplasmic RNA from cultured cells (Biotecx, Houston, Tex.); Biodyne Nylon membranes for Southern and Northern blots (Pall Biosupport, East Hills, N.Y.); nitrocellulose membranes for screening libraries (Schleicher & Schuell, Keene, N.H.); and Taq Dye primer and Taq dye-terminator cycle sequencing kits for fluorescent labeled automated DNA sequencing (Applied Biosystems, Foster City, Calif.). λUni-Zap (host strain XL1 Blue) human lung cDNA library and pBS(+) and pBluescript SK⁻ phagemid vectors were from Stratagene (La Jolla, Calif.); λgt11 (host strain Y1090) human kidney and bovine lung cDNA libraries; λEMBL-3A Sp6/T7 (host strain LE 392) bovine genomic library; and poly(A)⁺ RNA were from Clontech (Palo Alto, Calif.).

Example 2 Determination of the Amino Acid Sequence of Bovine Aspartoacylase Peptides

The amino terminal sequence of bovine brain aspartoacylase could not be obtained due to the autolysis of purified protein during storage. Purified aspartoacylase was digested with cyanogen bromide.sup.40 and peptides were fractionated on a 16.times.100 mm Mono Q column (FPLC system, Pharmacia LKB). Peptides were eluted with a 0-30% linear gradient of 1 M sodium chloride in buffer A (25 mM Tris.Cl pH 7.2 and 0.1% sodium azide), at a flow rate of 2 ml/min. The amino acid sequences of four peptides determined at a protein sequencing facility (Yale University, New Haven, Conn.) were as follows:

(SEQ ID NO: 13) CN8.1: LENSTEIQRTGLEVKPFITNPRAVKK; (SEQ ID NO: 14) CN8.2: KPLIPXDPVFLTLDGKTISLGGDQTXYPXFXNEAAYY; (SEQ ID NO: 15) CN30: XKVDYPRNESGEISAIIHPKLQDQ; and (SEQ ID NO: 16) CN41: XXXALDFIXNFXEXKE.

Example 3 Preparation of Oligonucleotides; Reverse Transcription; PCR Amplification; DNA Probes

Oligonucleotides were synthesized by phosphoramidite chemistry on a 380B DNA Synthesizer (Applied Biosystems, Foster City, Calif.). First strand cDNA was synthesized by reverse transcription of 20 ng of Poly(A)⁺ RNA or 4 μg of cytoplasmic RNA with either oligo(dt)_(n) or a gene-specific primer under standard conditions suggested by the manufacturer. DNA amplification⁴¹ was carried out in DNA Thermal cycler Model 9600 (Perkin-Elmer Cetus, Norwalk, Conn.). Specific DNA sequences were amplified in 100 μl volumes with 20 ng of cloned or 500 ng of genomic DNA template according to the standard conditions suggested by the manufacturer. The PCR conditions were: 1 cycle of denaturation at 94° C. for 3 min, annealing for 30 sec at temperatures (T_(m)−4° C.) that were primer-dependant and extension at 72° C. for 1 min; followed by 27 cycles of denaturation at 94° C. for 30 sec, annealing for 30 sec and extension at 72° C. for 30 sec. The last step was extension at 72° C. for 7 min. The tubes were chilled to 4° C. until further analysis. For SSCP⁴² and restriction digestion analysis of mutant alleles, PCR was carried out similarly except that 1 μCi of α-[³²P] dCTP was included in the PCR reaction mixture.

Small DNA fragments of less than 200 bp were labeled with ³²P by PCR amplification of the desired DNA sequences using α-[³²P] dNTP's. DNA fragments bigger than 200 bp were labeled by the random primer method⁴³ following the conditions suggested by the manufacturer. The specific activities of probes were 3-5×10⁸ cpm/μg DNA.

Example 4 Isolation of cDNA Clone, and Determination and Analysis of the Nucleotide Sequence

The first strand bovine cDNA was synthesized by reverse transcription (RT) of bovine kidney poly(A)⁺ RNA with oligo(dt)₂₀. The bovine aspartoacylase-specific coding sequences were amplified by polymerase chain reaction (PCR) using first strand cDNA as the template and CN30 peptide-based primers

-   CD5 (AAA/GGTIGAC/TTAC/TCCIIGIAA;) and -   CD8 (TGA/GTCC/TTGIAIC/TTTIGGA/GTG).

The cDNA fragment thus amplified was 69 bp long, which is the size expected from the CN30 peptide. The ORF of this fragment predicted the amino acid sequence of CN30 peptide. The 69 bp fragment was used as a probe to screen .lamda.gt11 bovine lung cDNA library. One cDNA clone, .lamda.ABL2, was isolated. The insert in .lamda.ABL2 had a single 839 bp long ORF. The amino acid sequence predicted by the ORF of .lamda.ABL2 insert contained the CN8.1, CN8.2, CN30, and CN41 peptide sequences described earlier. However, the cDNA clone was truncated at the 5′ and 3′ termini. The sequences downstream of the 3′ termini of .lamda.ABL2 insert were cloned by RT-PCR amplification of bovine kidney poly(A).sup.+RNA using oligo(dt).sub.20 and the bovine aspartoaqase cDNA specific primer CD48-1 (CCGTGTACCCAGTGTT; SEQ ID NO: 19).

A unique 770 bp fragment was amplified that overlapped with the 3′ sequence of λABL2 insert. The insert from λABL2 was used to screen bovine liver genomic library cloned in λEMBL3A vector according to the standard conditions^(44,45). Limited nucleotide sequence of genomic clones identified the missing 5′ coding and non-coding sequences of bovine aspartoacylase cDNA.

Bovine cDNA (data not presented), was next used for isolation of human ASP cDNA clones. Human cDNA libraries were screened and the isolated clones analyzed by the methods described earlier or according to the standard protocols^(44,45). The human lung aspartoacylase cDNA was rescued from λUni-Zap human lung cDNA clone by co-transfection with helper phage R408 into XL-1 Blue strain of E. coli according to the protocol suggested by the manufacturer. The rescued recombinant pHLASP was transfected into E. coli (XLI Blue strain). Large scale recombinant phagemid DNA were purified on cesium chloride gradients⁴⁵.

The nucleotide sequence of double stranded plasmid and amplified DNA fragments was determined by the dideoxy chain termination method⁴⁶. M13 universal/reverse and T3/T7 primers, or dideoxy NTP's, tagged with fluorescent dyes, were used for sequencing both strands of DNA fragments on an automated 373A DNA sequencer (Applied Biosystems, Foster City, Calif.). Fluorescent DNA sequencing was carried out with DNA sequencing kits and used according to the protocols suggested by the manufacturer.

Sequences were analyzed with Lasergene software package for DNA analysis from DNAstar (Madison, Wis.).

Example 5 Analysis of RNA

Cytoplasmic RNA was prepared from cultured cell lines⁴⁷ using a RNAZOL B kit for isolation of RNA (Biotecx, Houston, Tex.). Two to three μg of poly(A)⁺ RNA and 4.5 μg of RNA markers (Promega) were denatured with formamide. The denatured RNA was fractionated on a 1% agarose gel in formaldehyde containing buffer. The RNA was transferred overnight onto a nylon membrane. The blots were baked in a vacuum oven at 80° C. for 90 min, hybridized, and then washed under stringent conditions and autoradiographed⁴⁵.

Example 6 Expression of Aspartoacylase by Human Asp cDNA Clone pHLASP

The E. coli (XLI Blue strain) transformed with recombinant pHLASP or wild type pBluescript SK⁻ phagemid were grown overnight in 15 ml of Luria broth containing glucose (0.1%) and ampicillin (50 μg/ml) in the absence or presence of 20 mM IPTG. The bacteria were harvested, treated with 500 μL of 0.05 mg/ml lysozyme in 25 mM Tris.Cl pH 8.0, 10 mM EDTA and 50 mM glucose for 10 min at ambient temperature. The treated bacteria were diluted with ice cold 1.5 ml of 50 mM Tris.Cl, pH 8.0, 0.01% β-mercaptoethanol and 0.01% sodium azide and sonicated by three 10 sec bursts in ice cold conditions. The protein concentration in the bacterial sonicates was determined⁴⁸. Aspartoacylase assays were carried out in duplicate with 450 μg protein of bacterial sonicate under standard incubation conditions described elsewhere¹⁶. Controls lacking substrate or enzyme during the incubation were run simultaneously to account for background absorption in each assay. One mU of enzyme activity is defined as 1 nanomole of aspartate released/min of incubation time.

Example 7 Mutation Analysis

Cytoplasmic RNA (4 μg) from cultured fibroblast of normal controls, probands and their family members was reverse transcribed with

-   HKRT1 (AACCCTACTCTTAAGGAC; SEQ ID NO: 5).     Aspartoacylase specific coding sequences were amplified by PCR with -   HASP9 (CTTCTGAATTGCAGAAATCA; SEQ ID NO: 20) and -   HASPC7 (GTAAGACACCGTGTAAGATG; SEQ ID NO: 21)     primers. The full length coding sequence thus amplified was used as     template to amplify 200 to 300 bp overlapping cDNA fragments and     nucleotide sequence was determined. For a854>c point mutation     analysis, a 312 bp fragment was amplified with -   HASP14F (F→CCGGGATGAAAATGGAGAA; SEQ ID NO: 6) and -   HASPC7R (R→ACCGTGTAAGATGTAAGC; SEQ ID NO: 7)     primers. The prefix F and R in these oligos stand for M13 universal     and reverse primer tags, that allowed determination of nucleotide     sequence using fluorescent tagged M13 primes.

For SSCP and restriction digestion analysis, the 237 bp cDNA fragment with a854>c mutation was amplified in presence of α-[³²P] dCTP using

-   HASPG5 (AGGATCAAGACTGGAAACC; SEQ ID NO: 8) and -   HASPC7 (GTAAGACACCGTGTAAGATG; SEQ ID NO: 9)     primers. The analysis for SSCP in the 237 bp amplified cDNA     fragments was carried out in 40 cm long, 5% polyacrylamide gels in     1×TBE and 5% glycerol⁴². Electrophoresis was carried out at 7.5     Watts at ambient temperature for 16-18 h, and the gel was     autoradiographed. The a854>c mutation was also analyzed by     restriction digestion of 237 bp cDNA fragment with Eag I or Not I.     Following electrophoresis of the digest on native 5% polyacrylamide     gels in 1.times.TAE, the gel was autoradiographed.

Part II: Results Example 8 Isolation and Characterization of Human ASP cDNA

Human aspartoacylase specific coding sequences were amplified by RT-PCR of human kidney poly(A)⁺ RNA using oligo (dt)¹⁶ for first strand cDNA synthesis followed by PCR using bovine cDNA-based primers

-   CD56I (GGG/ATAIACIGTT/CTGG/ATCICCICC) and -   CD59I (CCIA/CGIGCIGTIAAA/GAAA/GTG) (data not shown).

A specific 676 bp cDNA fragment was amplified and found to have 90% identity to the corresponding region of the bovine ASP cDNA. The 676 bp partial human cDNA was used as probe to screen human lung .lamda.Uni-Zap and human kidney .lamda.gt11 cDNA libraries. This resulted in the isolation of several overlapping clones. Three of the clones with largest insert of 1.45 kb, also had identical terminal sequences. One of these, .lamda.gt11 HK5-1 was isolated from human kidney library and two clones .lamda.Uni-Zap HL 1 and two were isolated from the human lung library. The recombinant pHLASP was excised from .lamda.Uni-Zap HL1 clone. The nucleotide and the predicted amino acid sequence of pHLASP is shown in FIG. 1 (SEQ ID NO: 1).

The human ASP cDNA is 1,435 bp with 158 bp 5′ and 316 bp 3′ untranslated sequence. The isolated cDNA has 18 bases long poly(A) tail. A polyadenylation signal “aataaa” is found 48 bases upstream from the poly(A) addition site. Another consensus polyadenylation signal sequence “tataaa” is present 23 bases upstream from the poly(A) addition site. The position of “tataaa” is within the suggested location of 10-30 bases upstream from the poly(A) addition site^(17,18). Human and bovine ASP encoded transcripts and proteins do not match any known sequences in the databases.

The open reading frame (ORF) in human ASP cDNA predicted 313 amino acid long protein that is 92% identical to bovine ASP encoded protein (see FIG. 2). The molecular weight is estimated to be 36 kD. The predicted protein sequence has potentially one “N” glycosylation and 7 phosphorylation sites. The amino acid sequence motifs GGTHGNE (SEQ ID NO: 10), DCTV (SEQ ID NO: 24) and VNEAAYY (SEQ ID NO: 11) identified in both proteins, are similar to the consensus sequences GXXHG/AXE/D (SEQ ID NO: 25), DXXFN (SEQ ID NO: 26) and VXEXXXY (SEQ ID NO: 27) involved in the catalysis by esterasee¹⁹.

Example 9 Tissue Distribution and Size of Aspartoacylase Transcripts

Human poly(A)⁺ RNA, 2 μg each from various tissues, were analyzed by Northern blot analysis (FIG. 3). The poly(A)⁺ RNA from human liver gave a single band of 1.44 kb, whereas that from other human tissues tested gave two bands of 1.44 and 5.4 kb. The 1.44 kb faster moving band was similar in size to the 1.435 kbp human ASP cDNA. It appears that human brain expresses a relatively higher proportion of the larger transcript, as compared to relative amounts of the two transcripts in each of the tissues analyzed. The intensity of signals for both bands was highest in human skeletal muscles, followed by kidney and brain.

Example 10 Expression of Aspartoacylase Activity in Human Lung cDNA

The orientation of human ASP cDNA (pHLASP) cloned in pBluescript SK⁻ phagemid vector is shown in FIG. 4. The cDNA was cloned as an Eco RI and Xho I insert in pBluescript SK⁻ phagemid in 5′→3′ direction. The transcription of human ASP cDNA, driven by LACZ promoter, was studied in the absence and presence of the LACZ inducer isopropylthio-β-D-galactoside (IPTG) in E. coli (XL1 Blue strain). The mean aspartoacylase activity expressed by the pHLASP construct was 0.111, (range 0.044-0.175), mU/mg protein in the absence of IPTG. The activity increased 4-fold to 0.436 (range 0.223-0.622) mU/mg protein when cultures were grown in the presence of 20 mM IPTG. The level of activity expressed by pHLASP was more than 2 orders of magnitude higher than the mean residual activity of 0.019 (range 0.000-0.043) mU/mg protein observed with wild type pBluescript SK⁻ in the presence of IPTG. These results demonstrate that human ASP cDNA codes for aspartoacylase.

Example 11 Determination of a Missense Mutation in Human ASP cDNA from Patients with CD

The ASP encoded transcripts were analyzed from family members of 17 unrelated pedigrees of Ashkenazi Jewish background. Representative nucleotide sequence data for mutation analysis is shown in FIG. 5. A base change a854>c was identified in patients with CD. Both parents of a854>c homozygous patients were carriers for this mutation. Normal controls and non-carrier sibling of patients with CD did not have the a854>c base change in their ASP encoded transcript. The a854>c base change would alter the E285 codon in aspartoacylase and result in E285>A missense mutation.

The a854>c base change creates recognition sequences for Eag I and Not I restriction endonuclease in the mutant allele. The mutation was analyzed in an amplified 237 bp cDNA fragment for single strand conformation polymorphism (SSCP) and by digestion with restriction endonuclease Eag I. Typical mutation analysis profile from three representative pedigrees are shown in FIG. 6. Individuals homozygous, heterozygous or non-carriers for a854>c mutation could be differentiated by SSCP analysis (see FIG. 6, Panel A). Following digestion of the 237 bp fragment with Eag I (FIG. 6, Panel B), probands homozygous for the a854>c point mutation produced two restriction fragments of 125 and 112 bp; obligate carriers and heterozygotes had an undigested 237 bp fragment and two restriction fragments of 125 and 112 bp, while normal controls and non-carriers for a854>c point mutation had only the 237 bp fragment. The a854>c base mutation was observed in 85% (29 out of 34) of the Canavan alleles and is inherited as a Mendelian recessive trait. Of the 17 probands, 12 were found to be homozygous and 5 were heterozygous for this mutation. In the 5 compound heterozygote patients with CD, the mutation on a second Canavan allele was further investigated. The a854>c base change was not observed in any of 84 normal individuals analyzed so far.

Example 12 Additional Mutations Identified

In addition to the major mutation present in 85% of the Canavan patients and carriers, two other mutations were identified using similar analyses.

One is a c693>a mutation, which results in the codon change TAC>TAA, which results in a translation error of Y231>X; thus, this mutation causes premature termination of the polypeptide chain at the location where a tyrosine residue is supposed to be. This is a “nonsense” mutation.

Another allele which has been identified is a c914>a change, which results in the codon change GCA>GAA, which in turn results in the missense mutation A305>E, substituting a glutamic acid for an alanine residue.

The preceding examples can be repeated with similar success by substituting the generically or specifically described reactants and/or operating conditions of this invention for those used in the preceding examples.

From the foregoing description, one skilled in the art can easily ascertain the essential characteristics of this invention, and without departing from the spirit and scope thereof, can make various changes and modifications of the invention to adapt it to various usages and conditions.

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What is claimed is:
 1. A kit for assaying for the presence of a human aspartoacylase gene by immunoassay, comprising: (a) an antibody which specifically binds to a gene product of the human aspartoacylase gene; (b) a reagent means for detecting binding of the antibody to the gene product; wherein the antibody and reagent means are each present in amounts effective to perform the immunoassay.
 2. The kit of claim 1, wherein said reagent means for detecting binding comprises fluorescence detection, radioactive decay detection, enzyme activity detection or colorimetric detection.
 3. The kit of claim 2, wherein said aspartocylase gene is wild-type human aspartoacylase gene.
 4. The kit of claim 2, wherein said aspartoacylase gene is a mutant human aspartoacylase gene.
 5. The kit of claim 1 wherein said antibody is a monoclonal antibody that is specific for said gene product of human aspartoacylase gene.
 6. The kit of claim 1, wherein said antibody molecule comprises an F′(ab)₂ fragment which binds to said gene product of human aspartoacylase gene.
 7. An immunologically active anti-aspartoacylase antibody which is specific for a human aspartoacylase polypeptide, wherein said aspartoacylase poplypeptide is capable of hydrolyzing N-acetyl-aspartic acid to aspartate and acetate.
 8. The antibody of claim 7, which is a monoclonal antibody that is specific for said wild type aspartoacylase.
 9. The antibody of claim 7, wherein said antibody molecule comprises an F′(ab)₂ fragment which binds to said wild type aspartoacylase.
 10. An immunologically active anti-aspartoacylase antibody which is specific for a mutant aspartoacylase polypeptide having either an altered ability to hydrolyze N-acetyl-aspartic acid to aspartate and acetate, as compared with a wild-type human aspartoacylase, or incapable of hydrolyzing N-acetyl-aspartic acid to aspartate and acetate, and comprising the polypeptide sequence set forth in SEQ ID NO: 2 or a wild-type human aspartoacylase, except that said sequence has one or more of the following amino acid substitutions: E285>A, Y231>X, and/or A305>E, whereby E is glutamate, A is alanine, Y is tyrosine, and X is any naturally-occurring amino acid.
 11. The antibody of claim 10, which is a monoclonal antibody that is specific for said mutant aspartoacylase.
 12. The antibody of claim 10, wherein said antibody molecule comprises an F′(ab)₂ fragment which binds to said mutant aspartoacylase.
 13. A hybridoma which produces a monoclonal antibody of claim 8, wherein said antibody is specific for a wild-type aspartoacylase polypeptide.
 14. The hybridoma of claim 13 wherein said antibody is specific for said wild-type human aspartoacylase polypeptide.
 15. A hybridoma which produces a monoclonal antibody of claim 11, wherein said antibody is specific for a mutant aspartoacylase polypeptide.
 16. The hybridoma of claim 15 wherein said antibody is specific for said mutant aspartoacylase polypeptide having either an altered ability to hydrolyze N-acetyl-aspartic acid to aspartate and acetate, as compared with a wild-type human aspartoacylase, or incapable of hydrolyzing N-acetyl-aspartic acid to aspartate and acetate, and comprising the polypeptide sequence set forth in SEQ ID NO: 2 or wild-type human aspartoacylase, except that said sequence has one or more of the following amino acid substitutions: E285>A, Y231>X, and/or A305>E, wherein E is glutamate, A is alanine, Y is tyrosine, and X is any naturally-occurring amino acid.
 17. An antibody which is specific for human aspartoacylase polypeptide, wherein said polypeptide comprises the sequence set forth in SEQ ID NO: 2 or a variant of SEQ ID NO: 2 having at least one amino acid substitution which is E285>A, Y231>X, and/or A305>E, whereby E is glutamate, A is alanine, Y is tyrosine, and X is any naturally-occurring amino acid. 